Laccase-Treated Polystyrene Surfaces with Caffeic Acid, Dopamine, and L-3,4-Dihydroxyphenylalanine Substrates Facilitate the Proliferation of Melanocytes and Embryonal Carcinoma Cells NTERA-2

Author:

Li Hanluo12ORCID,Wilhelm Martin3,Baumbach Christina Marie4,Hacker Michael C.56ORCID,Szardenings Michael7ORCID,Rischka Klaus8ORCID,Koenig Andreas9ORCID,Schulz-Kornas Ellen10ORCID,Fuchs Florian9,Simon Jan Christoph11ORCID,Lethaus Bernd2ORCID,Savković Vuk2ORCID

Affiliation:

1. National “111” Center for Cellular Regulation and Molecular Pharmaceutics, Hubei Provincial Key Laboratory of Industrial Microbiology, Sino-German Biomedical Center, Hubei University of Technology, Wuhan 430068, China

2. Department of Cranial Maxillofacial Plastic Surgery, University Hospital Leipzig, 04103 Leipzig, Germany

3. Department of Ear, Nose and Throat Diseases, and Head and Neck Surgery, University of Greifswald, 17475 Greifswald, Germany

4. Julius-Bernstein-Institute of Physiology, Martin-Luther-University of Halle-Wittenberg, 06108 Halle, Germany

5. Institute of Pharmaceutic Technology and Biopharmaceutics, Department of Pharmacy, Math.-Nat. Faculty, Heinrich-Heine-Universität Düsseldorf, 40204 Düsseldorf, Germany

6. Institute for Pharmacy, Faculty of Medicine, Leipzig University, Eilenburger Straße 15 A, 04317 Leipzig, Germany

7. Fraunhofer Institute for Cell Therapy and Immunology IZI, 04103 Leipzig, Germany

8. Fraunhofer Institute for Manufacturing Technology and Advanced Materials IFAM, 28359 Bremen, Germany

9. Polyclinic for Dental Prosthetics and Material Sciences, University Hospital Leipzig, 04103 Leipzig, Germany

10. Department of Cariology, Endodontology and Periodontology, University Hospital Leipzig, 04103 Leipzig, Germany

11. Clinic for Dermatology, Venereology and Allergology, University Hospital Leipzig, 04103 Leipzig, Germany

Abstract

This study presents the effects of treating polystyrene (PS) cell culture plastic with oxidoreductase enzyme laccase and the catechol substrates caffeic acid (CA), L-DOPA, and dopamine on the culturing of normal human epidermal melanocytes (NHEMs) and human embryonal carcinoma cells (NTERA-2). The laccase–substrate treatment improved PS hydrophilicity and roughness, increasing NHEM and NTERA-2 adherence, proliferation, and NHEM melanogenesis to a level comparable with conventional plasma treatment. Cell adherence dynamics and proliferation were evaluated. The NHEM endpoint function was quantified by measuring melanin content. PS surfaces treated with laccase and its substrates demonstrated the forming of polymer-like structures. The surface texture roughness gradient and the peak curvature were higher on PS treated with a combination of laccase and substrates than laccase alone. The number of adherent NHEM and NTERA-2 was significantly higher than on the untreated surface. The proliferation of NHEM and NTERA-2 correspondingly increased on treated surfaces. NHEM melanin content was enhanced 6-10-fold on treated surfaces. In summary, laccase- and laccase–substrate-modified PS possess improved PS surface chemistry/hydrophilicity and altered roughness compared to untreated and plasma-treated surfaces, facilitating cellular adherence, subsequent proliferation, and exertion of the melanotic phenotype. The presented technology is easy to apply and creates a promising custom-made, substrate-based, cell-type-specific platform for both 2D and 3D cell culture.

Funder

Department of Cranial Maxillofacial Plastic Surgery, University Clinic Leipzig, Germany, Saxon Ministry of Science and Fine Arts

German Research Council (DFG) SFB TRR 67 B12

Collaborative Grant-in-Aid of the HBUT National “111” Center for Cellular Regulation and Molecular Pharmaceutics

IZI-IFAM collaborative Project ZELLFIX supported by the Fraunhofer-Gesellschaft

Publisher

MDPI AG

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